TGF-β_1成熟肽基因克隆及在大肠杆菌中表达  被引量:1

CONSTRUCTION OF TGF-β_1 MATURE PEPTIDE GENE AND ITS EXPRESSION IN ESCHERICHIA COLI

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作  者:孙大铭[1] 侯树勋[1] 杜桂鑫[2] 童贻刚[2] 付小兵[1] 

机构地区:[1]解放军第304医院 [2]军事医学科学院微生物研究所

出  处:《解放军医学杂志》2002年第5期434-436,共3页Medical Journal of Chinese People's Liberation Army

基  金:国家 973项目资助课题 (编号G1 9990 542 0 4 )

摘  要:为在原核细胞中表达TGF β1单体蛋白 ,用基因重组技术构建pBV2 2 0 TGF β和 pQE TGF β两种原核表达载体 ,分别在M15和DH5α大肠杆菌中进行表达 ,然后利用SephacrylS 10 0凝胶层析及Ni+ NTA琼脂柱纯化TGF β1单体。经酶切鉴定及测序结果证明pBV2 2 0和pQE30载体上成功地插入了TGF β1成熟肽基因片段。pBV2 2 0 TGF β和pQE TGF β两种原核表达载体在大肠杆菌中均得到了高效表达 ,表达量约占全菌蛋白的 15 %和 2 0 % ,表达的TGF β1单体蛋白经纯化后进行SDS PAGE电泳 ,均显示了一条蛋白带 ,分子量分别为 13kD和 15kD左右。To further understand the function and biological activity of TGF β 1, and to provide the basis for the production of biologically active TGF β 1 protein, TGF β 1 cDNA was cloned into procaryotic expression vectors--pBV220 and pQE30, and the monomeric form of the recombinant TGF β 1expressed in E.coli DH5α and M15. Sephacryl S 100 HR and Ni + NTA agarose column were used to purify the TGF β 1 protein. With digestion of the enzymes and sequencing, TGF β 1 mature peptide gene was inserted into procaryotic expression vectors--pBV220 and pQE30. After purified, the expressed products of two plasmids in E.coli showed a single protein on SDS--PAGE, and their expression levels were about 15% and 20% of the total bacterial protein. The construction of recombinant plasmids and preparation of the monomeric protein of TGF β 1 lay a solid foundation for further studying the function of TGF β 1 and producing biologically active TGF β 1 protein.

关 键 词:转化生长因子Β 基因重排 基因表达 质粒 大肠杆菌 

分 类 号:Q782[生物学—分子生物学]

 

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